Factor V (Quebec): a bleeding diathesis associated with a qualitative platelet Factor V deficiency.

Tracy, Paula B.; Giles, Alan R.; Mann, Kenneth G.; Eide, Lisa; Hoogendoorn, Hugh; Rivard, Georges E.

doi:10.1172/jci111531

Cited by 130 publications

(89 citation statements)

References 31 publications

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“…One hundred twenty-seven relatives within 2 families with known inheritance of QPD 11,12 participated in the study. When information for the updated pedigree was acquired, a common ancestor was identified, allowing the 2 pedigrees to be merged ( Figure 1).…”

Section: Resultsmentioning

confidence: 99%

“…[11][12][13][14][15][16] The cases initially reported had moderate to severe delayed bleeding problems that responded to treatment with fibrinolytic inhibitors. [11][12][13] Although these bleeding problems were initially attributed to a deficiency of functional platelet factor V, and hence the designation factor V Quebec, the disorder is now known to be associated with a complex spectrum of unique platelet and fibrinolytic abnormalities that include increased megakaryocyte expression and storage of urokinase-type plasminogen activator (u-PA), ␣-granule protein degradation associated with intraplatelet generation of plasmin, normal to increased plasma u-PA without increased plasma D-dimers, normal to reduced platelet counts, absent platelet aggregation responses to 6 M epinephrine, and normal to abnormal aggregation responses to collagen and adenosine diphosphate (ADP). [11][12][13][14][15][16][17] Access to affected and unaffected individuals within families with QPD, the large pedigree sizes, and definitive blood tests for QPD [12][13][14] provided a unique opportunity to investigate bleeding risks for an autosomal dominant trait and to gather data on responses of QPD bleeding to fibrinolytic inhibitor therapy.…”

Section: Introductionmentioning

confidence: 99%

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Bleeding risks associated with inheritance of the Quebec platelet disorder

McKay

Derome

Haq

et al. 2004

Blood

197

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Quebec platelet disorder (QPD) is an autosomal dominant bleeding disorder associated with increased urokinase-type plasminogen activator in platelets and ␣-granule protein degradation. To determine bleeding risks and common manifestations of QPD, a history questionnaire was developed and administered to 127 relatives in a family with QPD. Data entry was done blinded to affected and unaffected status, determined by assays for platelet urokinase-type plasminogen activator (u-PA) and fibrinogen degradation. Odds ratios (ORs), with 95% confidence intervals (CIs), were determined for items queried. Summative bleeding scores for each individual were calculated using items with OR more than 1. Mean ages (34 years; range, 1-89 years) were similar for affected (n ‫؍‬ 23) and unaffected (n ‫؍‬ 104) family members. Affected individuals had higher mean bleeding scores (P < .0001) and a much higher likelihood (OR > 20) of having bleeding that led to lifestyle changes, bruises that spread lower or as large or larger than an orange or both, joint bleeds, bleeding longer than 24 hours after dental extractions or deep cuts, and received or been recommended other treatments (fibrinolytic inhibitors) for bleeding. Individuals with QPD and exposure(s) to hemostatic challenges had experienced excessive bleeding only when fibrinolytic inhibitors had not been used. These data illustrate that QPD is associated with increased risks of bleeding that can be modified by fibrinolytic inhibitors.

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Section: Resultsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Bleeding risks associated with inheritance of the Quebec platelet disorder

McKay

Derome

Haq

et al. 2004

Blood

197

View full text Add to dashboard Cite

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“…1,[4][5][6] This disorder was initially designated as factor V Quebec because of the abnormalities found in platelet factor V of these patients. 7 Two families from Quebec have been identified with this condition, which is now known to be associated with other platelet abnormalities that include reduced to low-normal platelet counts, proteolytic degradation of soluble and membrane proteins stored in platelet ␣-granules, an apparent quantitative deficiency of the ␣-granule protein multimerin, and defective aggregation with epinephrine. 1,[4][5][6]8 Although patients with the QPD have elevated levels of fibrinogen degradation products (FDPs) in their serum (because of platelet fibrinogen degradation), their plasma contains normal amounts of FDPs and D-dimers.…”

Section: Introductionmentioning

confidence: 99%

Platelets from patients with the Quebec platelet disorder contain and secrete abnormal amounts of urokinase-type plasminogen activator

Kahr

Zheng

Sheth

et al. 2001

Blood

112

142

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The Quebec platelet disorder (QPD) is an autosomal dominant platelet disorder associated with delayed bleeding and ␣-granule protein degradation. The degradation of ␣-granule, but not plasma, fibrinogen in patients with the QPD led to the investigation of their platelets for a protease defect. Unlike normal platelets, QPD platelets contained large amounts of fibrinolytic serine proteases that had properties of plasminogen activators. Western blot analysis, zymography, and immunodepletion experiments indicated this was because QPD platelets contained large amounts of urokinase-type plasminogen activator (u-PA) within a secretory compartment. u-PA antigen was not increased in all QPD plasmas, whereas it was increased more than 100-fold in QPD platelets (P < .00009), which contained increased u-PA messenger RNA. Although QPD platelets contained 2-fold more plasminogen activator inhibitor 1 (PAI-1) (P < .0008) and 100-fold greater u-PA-PAI-1 complexes (P < .0002) than normal platelets, they contained excess u-PA activity, predominantly in the form of two chain (tcu-PA), which required additional PAI-1 for full inhibition. There was associated proteolysis of plasminogen in QPD platelets, to forms that comigrated with plasmin. When similar amounts of tcu-PA were incubated with normal platelet secretory proteins, many ␣-granule proteins were proteolyzed to forms that resembled degraded QPD platelet proteins. These data implicate u-PA in the pathogenesis of ␣-granule protein degradation in the QPD. Although patients with the QPD have normal to increased u-PA levels in their plasma, without evidence of systemic fibrinogenolysis, their increased platelet u-PA could contribute to bleeding by accelerating fibrinolysis within the hemostatic plug. QPD is the only inherited bleeding disorder in humans known to be associated with increased u-PA. IntroductionCongenital platelet disorders are usually associated with defective primary hemostasis. [1][2][3] The Quebec platelet disorder (QPD) is an autosomal dominant platelet disorder that has unusual clinical features: it is associated with moderate to severe delayed bleeding, that typically begins 12 to 24 hours after surgery or trauma, and its hemorrhagic manifestations can be controlled with fibrinolytic inhibitors but not with platelet transfusions. 1,[4][5][6] This disorder was initially designated as factor V Quebec because of the abnormalities found in platelet factor V of these patients. 7 Two families from Quebec have been identified with this condition, which is now known to be associated with other platelet abnormalities that include reduced to low-normal platelet counts, proteolytic degradation of soluble and membrane proteins stored in platelet ␣-granules, an apparent quantitative deficiency of the ␣-granule protein multimerin, and defective aggregation with epinephrine. 1,[4][5][6]8 Although patients with the QPD have elevated levels of fibrinogen degradation products (FDPs) in their serum (because of platelet fibrinogen degradation), their plasma contains normal amo...

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“…Its paramount importance in the maintenance of normal hemostasis, when compared with that of plasma-derived FVa, has been demonstrated in several clinical studies. Individuals expressing substantially decreased levels of FV in their platelets exhibit a life-threatening bleeding diathesis despite their expression of relatively normal levels of plasma-derived FV (4). An individual with an antibody that neutralized greater than 99% of the plasmaderived FV pool endured surgical challenge as the antibody was without effect on platelet-derived FV/Va, indicating that the platelet stores of FV/Va were sufficient to maintain normal hemostasis (11).…”

mentioning

confidence: 99%

Unique in Vivo Modifications of Coagulation Factor V Produce a Physically and Functionally Distinct Platelet-derived Cofactor

Gould¹,

Silveira²,

Tracy

2004

Journal of Biological Chemistry

105

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Platelet-and plasma-derived factor Va (FVa) serve essential cofactor roles in prothrombinase-catalyzed thrombin generation. Platelet-derived FV/Va, purified from Triton X-100 platelet lysates was composed of a mixture of polypeptides ranging from ϳ40 to 330 kDa, mimicking those visualized by Western blotting of platelet lysates and releasates with anti-FV antibodies. The purified, platelet-derived protein expressed significant cofactor activity such that thrombin activation led to only a 2-3-fold increase in cofactor activity yet expression of a specific activity identical to that of purified, plasma-derived FVa. Physical and functional differences between the two cofactors were identified. Purified, platelet-derived FVa was 2-3-fold more resistant to activated protein C-catalyzed inactivation than purified plasma-derived FVa on the thrombin-activated platelet surface. The heavy chain subunit of purified, plateletderived FVa contained only a fraction (ϳ10 -15%) of the intrinsic phosphoserine present in the plasma-derived FVa heavy chain and was resistant to phosphorylation at Ser 692 catalyzed by either casein kinase II or thrombin-activated platelets. MALDI-TOF mass spectrometric analyses of tryptic digests of platelet-derived FV peptides detected an intact heavy chain uniquely modified on Thr 402 with an N-acetylglucosamine or N-acetylgalactosamine, whereas Ser 692 remained unmodified. N-terminal sequencing and MALDI-TOF analyses of plateletderived FV/Va peptides identified the presence of a fulllength heavy chain subunit, as well as a light chain subunit formed by cleavage at Tyr 1543 rather than Arg 1545 accounting for the intrinsic levels of cofactor activity exhibited by native platelet-derived FVa. These collective data are the first to demonstrate physical differences between the two FV cofactor pools and support the hypothesis that, subsequent to its endocytosis by megakaryocytes, FV is modified to yield a platelet-derived cofactor distinct from its plasma counterpart.Factor Va (FVa), 1 a heterodimeric protein composed of heavy chain (105 kDa) and light chain (74 kDa) subunits, is formed by limited proteolysis of factor V (FV) (1). In normal hemostasis, FVa functions as a non-enzymatic cofactor of the prothrombinase complex, which consists of a 1:1 stoichiometric and Ca 2ϩ -dependent complex of the serine protease factor Xa and FVa, bound to the membrane of appropriately activated platelets, and catalyzes the proteolytic conversion of prothrombin to thrombin (2). When incorporated into the prothrombinase complex, the catalytic activity of factor Xa is increased by approximately 5 orders of magnitude, and FVa contributes substantially to this increase (3). Removal of FVa from the prothrombinase complex results in a 10,000-fold decrease in the rate of thrombin generation (3), the physiologic effect of which is demonstrated in the bleeding diatheses expressed by FV-deficient individuals (4 -8)Factor V circulates in two pools in whole blood. The majority (75-80%) is found in the plasma as an inactive, singl...

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Factor V (Quebec): a bleeding diathesis associated with a qualitative platelet Factor V deficiency.

Cited by 130 publications

References 31 publications

Bleeding risks associated with inheritance of the Quebec platelet disorder

Bleeding risks associated with inheritance of the Quebec platelet disorder

Platelets from patients with the Quebec platelet disorder contain and secrete abnormal amounts of urokinase-type plasminogen activator

Unique in Vivo Modifications of Coagulation Factor V Produce a Physically and Functionally Distinct Platelet-derived Cofactor

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